Bio-Rad Nuvia™ cPrime™ Media User Manual

3

Section 3

Preparation

Nuvia™ cPrime™ media are supplied fully hydrated in 20% ethanol

as a 50% (v/v) slurry. For column packing, removal of the shipping

buffer is recommended. Small volumes of Nuvia cPrime media are

easily washed in a Büchner funnel with 4–5 volumes of packing

buffer. For large volume preparation, cycle through 3–4 settling and

decanting steps using the column packing buffer in the shipping

container.

Removal of fines from Nuvia cPrime media is not required. If, however,

particle fines have been generated during handling, resuspend the settled

media and remove any opaque or cloudy supernatant before resettling is

complete. Repeat several times until supernatant is clear.

Section 4

Column Packing

Nuvia™ cPrime™ media can be packed using standard column

packing methods. To pack columns for optimal operation, a

20–50% slurry volume is recommended.

Packing Small Columns
This slurry packing method was designed to pack Nuvia cPrime

media in a conventional laboratory scale column with an internal

diameter of 5–50 mm. All buffers should be degassed. Since a

relatively large volume of slurry is required, a packing reservoir

should be used.

1. Prepare degassed 1.0 M NaCl, 20–50 mM buffer salt (see

Table 2) referred to herein as the packing buffer.

2. Decant the shipping solution away from the resin bed as

outlined in Section 3, maintaining an approximate slurry

percentage of 50%.

3. After thorough buffer exchange, prepare an aliquot of Nuvia

cPrime media in a graduated cylinder to determine the slurry

percentage.

4. Seal the cylinder and rotate it to suspend the resin. Caution:

do not mix with a magnetic stir bar as damage may occur.

Larger amounts of slurry may be mixed with a low-shear

impeller at low to moderate speed.